Microbiological process for simultaneously 1-dehydrogenating and 16-hydroxylating a steroid



United States Patent 3,536,586 MICROBIOLOGICAL PROCESS FOR SIMULTA- NEOUSLY l-DEHYDROGENATING AND 16- HYDROXYLATING A STEROID Bong Kuk Lee, Old Bridge, Dewey D. Y. Ryu, North Brunswick, Richard W. Thoma, Somerville, and Patrick A. Diassi, Westfield, N.J., assignors to E. R. Squibb & Sons, Inc., New York, N.Y., a corporation of Delaware No Drawing. Filed Jan. 25, 1968, Ser. No. 700,345 Int. Cl. C07c 167/14 US. Cl. 195-51 3 Claims ABSTRACT OF THE DISCLOSURE This invention relates to a process for converting steroids by simultaneously adding an hydroxy group and dehydrogenating the 1,2-position in a mixed culture fermentation utilizing a species of Arthrobacter and an hydroxylating microorganism.

SUMMARY OF THE INVENTION The invention of the application is a process for treating a steroid, which is saturated in the 1,2-position of the A-ring and has a replaceable hydrogen in the 11,16,17 or 21-position, simultaneously with a microorganism of the genus Arthrobacter and with one or more of a hydroxylating microorganism in a mixed culture fermentation so that in the same operation a double bond is introduced into the 1,2-position and a hydroxy group is introduced into one or more of the 11,16,17 or 2l-positions. It has been found that the mixed culture enhances the results obtained in a fermentation with a dehydrogenator of the genus Arthrobacter.

Conversion of steroids is frequently effected by the action of microorganisms in a fermentation medium whereby functional groups are introduced into the steroid nucleus or other transformations take place. When several microbiological transformations have been utilized in the synthesis of steroids, particularly those involving different genera or species of organisms and involving various changes in the steroid structure, these have usually been proposed sequentially rather than simultaneously in the belief that competing reactions would render the action of the microorganism less specific and reduced the yield.

It has now been found that when dehydrogenating with a bacterial microorganism (or the active enzymes) of the genus Arthrobacter and hydroxylating with a mold or molds dehydrogenation and hydroxylation occur efficiently in a simultaneous reaction by contacting the steroid to be dehydrogenated and hydroxylated in a medium containing both the dehydrogenating and hydroxylating organisms. In the process of our invention combinations of organism and substrate are chosen so that the net result, in terms of overall efficiency of conversion of one steroid to another of greater value, is more efficient than are comparable processes in which the cultures are used separately or sequentially.

Among the known and valuable steroids which may be synthesized by the process of the invention are prednisolone, triamcinolone, dexamethasone, their 6u-fluoro analogs as well as 6u-methylprednisolone and the like.

Thus, for example, when a soybean medium containing 9a-fiuorohydrocortisone is simultaneously inoculated with the l-dehydrogenator A. simplex and the 16a-hydroxylator S. roseochromogenes under conditions of incubation normally used for 16-hydroxylation, that substance is completely converted to triamcinolone in 72 hours. In this medium S. roseochromogenes in pure culture normally converts about 300 gJml. of 9a-fiuorohydrocortisone to 9a-fluoro-l6a -hydroxyhydrocortisone is about 96 hours.

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Alone, A. simplex under these conditions effects l-dehydrogenation but also reduces the 20-keto group. In the combined, simultaneous fermentation process there is no evidence of ZO-dihydro products or of free 9a-fluoro-l6w hydroxyhydrocortisone. Thus, not only are the desirable reactions enhanced by physiological interaction of the organisms, but undesirable reactions are suppressed. More exactly, the actinomycete appears to repress, or prevent induction of the 20-keto-reductase of A. simplex, and at the same time the l6a-hydroxylating activity of S. roseochrom'ogenes is enhanced.

A different, but also advantageous type of interaction is observed when a cornsteep medium containing 16a-hydroxycortexolone 16,17 acetonide is inoculated with a fungus such as Curvulariw lunata or Absidia coerulea and bacterial species A. simplex. 1n cornsteep medium, induction of the l-dehydrogenating enzyme of A. simplex, when grown first in soybean meal medium, is repressed in pure culture. However, when A. co erulea or C. lunata is also present during the entire fermentation, induction of l-dehydrogenase of A. simplex occurs, i.e, the repression is relieved or counteracted by the metabolic activity of the fungus.

Species of the genus Arthrobacter, in addition to A. simplex, which effect the introduction of a double bond into the 1,2-position of the A-ring of a steroid (l-dehydrogenators) include globiformis, pascens, oxydans, aurescenJs, ureafaciens, tumescens, citreus, and terregens.

Microorganisms which effect the introduction of an hydroxy group into a position of the steroid nucleus having a replaceable hydrogen atom include Moi-hydroxylating species of the genera Streptomyces, especially S. roseochromogenes, Didymella or Pestalotia; 11p hydroxylating species of the genera Curvularia, especially C. lunata, Coniothyrium, especially, C. hellebori, Botrytis, Colletotrichum, especially C. phomoides, Cunninghamella, especially, C. blakesleeana, Rhodoseptoria, Pseudomonas or Pycnosporium; 11a and llfl-hydroxylating species of the genera Absidia, especially A. coerulea, Blakes lea, Choanephora, Circinella, Stachylidium, Thamnidium, especially, T. elegans, or Tieghemella; lla-hydroxylating species of the genus Aspergillus, especially, A. ochraceus, Bacillus, especially, B. cereus, Beauveria dactylium, Fusarium, Hormodendrum, Mucor, Rhizopus, especially, R. nigricans, Neurospora, Nigroospora or Penicillium; 17ahydroxylating species of the genera Tricothecium, especially T ricothecium roseum, Cladosporium, Leptosphaeria or Trichodema; 2l-hydroxylating species of the Wojnowicia, especially, W. graminis, Ophiobolus, especially, O. herpotrichus or H endersonia.

The combination of organisms may be composed of any ofthe above named l-dehydrogenating species of Athrobacter and one or more of the group of hydroxylators. The special advantage of the invention is derived from the fact that organisms properly selected, by interacting, perform better together than separately. The advantage is shown most strikingly in the combination of Arthrobacter simplex and Streptomyces roseochromogenes.

The inoculum for the mixed culture fermentation may be prepared by cultivating the given organism on media best adapted for growth of that particular organism. An agar slant culture may be used to provide surface growth to inoculate a shaken flask for further propagation of the microorganism according to the conventional techniques. Growth from the first or later member of a series of shaken flasks may then be used in the mixed culture fermentation.

Thus, for example, the composition of an agar medium suitable for the cultivation of bacteria such as A. simplex is as follows:

3 MEDIUM A G. Beef extract (Difco) 1.5 Yeast extract (Difco) 3.0 Peptone (Difco) 6.0 Dextrose 1.0

Distilled water q.s. 1 liter Autoclave minutes at 121 C.

Another agar medium adapted especially to the growth of actinomycetes such as S. roseochromogenes is:

MEDIUM B Agar (Difco) 20.0 Glucose 10.0 Yeast extract (Difco) 2.5 Potassium phosphate (dibasic) 1.0

Distilled water, 1 liter. Autoclave at 121 for 20 minutes.

A medium which may be used in the initial shaken flask stages when cultures of bacteria and actinomycetes are to be grown may 'be made as follows:

MEDIUM C Extracted soybean meal (Archer-Daniels-Midland) 15.0 Soybean oil 2.2 Glucose monohydrate 11.0 Calcium carbonate (technical) 2.5 Tap water q.s. 1.0 liter.

The mixed culture fermentation of this invention is carried out in a liquid culture medium containing conventional sources of carbohydrate, nitrogenous substances, inorganic salts and growth factors. The sources of carbohydrates include, for example, soybean meals, glucose, saccharose, molasses and the like. Nitrogenous substances include, for example, amino acids, casein hydrolysates, cereal grain meals, peptones, meat extracts, cornsteep liquor, and the like. Representative of the inorganic salts are magnesium sulfate, sodium acid phosphate and potassium phosphate (dibasic and monobasic). Growth factors may 'be added in pure form or may be obtained from yeast extract or trace impurities in the crude nitrogenous materials.

The steroid substrate to be converted may be added to the fermentation medium as a solution or suspension in water. Preferably a small amount of surface active agent such as Tween 80 is included in the solution or suspension. The amount of steroid substrate introduced into the fermentation medium may vary within rather broad limits but preferably it is in a proportion of about 0.2 to 2 grams/ liter.

Illustrative of the composition of the medium for mixed culture fermentation and one that is preferred for mixed culture fermentations with bacteria and actinomycetes is the following:

MEDIUM D Extracted soybean meal (ADM) 20.0 Glucose monohydrate 33.0 Calcium carbonate (technical) 7.5 Soybean oil 2.2 Potassium phosphate (dibasic) 1.0 Potassium phosphate (monobasic) 1.0

Tap water q.s. 1 liter. Autoclave at 121 C. for minutes.

A medium well suited for cultivation of fungi such as C. lunata or A. coerulea, as well as for A. simplex, when mixed c ltures of these are i t n d, is a f s 4 MEDIUM E Glucose 30.0 Soybean meal (staleys 4s) 20.0 Soybean oil 2.2 CaCO3 2-5 Distilled water q.s. 1 liter. Autoclave at 121 for 30 minutes.

A medium preferred for the final stage in mixed culture fermentations of fungi and bacteria is:

MEDIUM F Cornsteep liquor solids 3.0 .(NH )H PO 3-0 Yeast extract (Difco) 2.5 Glucose 10.0

Adjust to pH 1.0 Distilled water qs. 1 liter. Autoclave at 121 C. for 30 minutes.

About 1 to 20%, prefer-ably about 5% (VOL/vol.) of inoculum of each of the l-dehydrogenating species is used to inoculate the fermentation medium. The inoculation is best efitected as nearly simultaneously as possible although some interval between inoculation with the microorganisms is not deleterious in some cases so long as interaction between them occurs. For best results, the steroid too should be added substantially simultaneously.

It is also possible to introduce a portion of the steroid simultaneously with the microorganisms and then addition-a1 increments of the steroid as the reaction progresses.

After the two cultures and the steroid have been added to the medium, incubation is carried out under aerobic conditions (e.g., about 0.5-1.0 vol./vol./min.), preferably with agitation (e.g., about 400-600 r.p.m.). The fermentation may be carried out at a temperature within the range of about 15 to 45 C., preferably about 25 C.

The dehydration and hydroxylation are generally complete within a period of about 20 to 200 hours. Usually about 72 hours are sufiicient.

The product is separated from the fermentation medium by the conventional means of filtering ofi the solids and recovering the product from the filtrate by solvent extraction, selective precipitation or the like. Alternatively, whole broth may be contacted with a miscible or immiscible solvent prior to removal of solids by filtration or centrifuga-tion. Solids obtained by centrifugation or filtration, before or after contact with solvent, may be extracted further with acetone, methyl-isobutyl-ketone, or the like.

This method may be used to produce, for example, corticosteroids such as predisolone, triamcinolone, dexamethasone, 61x fiuorodexamethasone, 6a fluorotriamcinolone, 6oz fluorotriamcinolone acetonide, 6a methylprednisolone, and the like, as well as intermediates such as 1604 hydroxyprednisolone, 16a hydroxyprednisolone- 16,17 acetonide, 1 dehydro llu, l6u-dihydroxycortexolone, 16a hydroxyprednisolone, 1 dehydro 16-dehydro 110a hydrocortexone, 1 dehydro 11a,'16a-dihydroxycortexolone 16,17 acetonide, 16oz hydroxyprednisolone 16,17 acetonide, 6a fluoro-l6ot-methylprednisolone, and 6a fluoro 16cc methylprednisolone-16, 17-acetonide, which may be ultimately converted into such compounds.

Illustrative of the steroids which are saturated in the 1,2-position and have a replaceable hydrogen in the 11, 16,17 or 21-position and which may be subjected to dehydrogenation and hydroxylation by the process of this invention are the following: 9a fiuorohydrocortisone and 21-esters thereof such as fiuorohydrocortisone 21- acetone, 9a fluorohydrocortisone 2'1 hemisuccinate and the like, cortexolone, 16cc hydroxycortexolone, 16a-hydroxycortexolone 16,17 acetonide and ZI-esters thereof such as the acetate, hydrocortisone and 20-esters thereof such as hydrocortisone 21 acetate, 6m fluoro-16a-hydroxycortexolone 16,17 acetonide, 60c fluoro-16amethylcortexolone, 6a methylcortexolone, 16 dehydrocortexone, and 21-esters thereof such as acetate.

The mixed culture fermentation process of this invention, involving the use of a l-dehydrogenating species of the genus Arthrobacter and at least one hydroxylating organism simultaneously with the interaction of cultures and their enzymes during growth and enzyme formation in the presence of steroid, occurs in such a way that undesirable transformations are avoided and desirable enzymatic activities are enhanced. The resultant one-step conversion offers advantages over multistep processes not only in economy of material and time but also in the reduction of losses occurring in sequential recovery procedures.

The following examples are illustrative of the invention.

EXAMPLE 1 Surface growth from a -7 day old agar slant culture of Arthrobacter simplex ATTC No. 6946 grown on Medium A above is used to inoculate 50 ml. of Medium C above contained in a 250 ml. Erlenmeyer flask. The inoculated flask is placed for incubation at 25 C., and agitated at 280 r.p.m. in a circle of diameter 2 inches on a shaking machine. After 48 hours a (vol/vol.) transfer is made to another .250 ml. flask containing 50 ml. of Medium C. The second flask, after inoculation, is incubated under the same conditions as the first.

Proceeding on the same schedule as with the first culture, surface growth from a 5 day old agar slant culture grown on Medium B above of Streptomyces roseochromogenes ATCC No. 13,400 is transferred to 50 ml. of Medium C. contained in a 250 ml. Erlenmeyer flask. The flask medium is the same as that used for propagation of A. simplex in the first two flask stages.

The first shaken flask culture of S. roseochromogenes, inoculated as indicated, is incubated for 48 hours under conditions identical to those used for propagation of A. simplex. A second flask stage is inoculated by 10% (VOL/vol.) transfer, and incubation ofthe second flask is carried out as the first, for 48 hours. Thus, inoculum of the two cultures is ready for use at the same time.

Both cultures are used to inoculate 50 ml. portions of Medium D above. 5% (vol./vol.) inoculum of each species is used, and the inoculation is as nearly simultaneous as possible. Also at the same time a suspension of 9a-fluorohydrocortisone is added in aqueous suspension to provide 300 ,ug. of steroid/ml. of mixed culture broth. The suspension of steroid is prepared by adding finely powdered steroid to 0.01% aqueous Tween 80 to give 30 mg./ml., and autoclaving for minutes at 121 C.

After the two cultures and steroid suspension are added to the fermentation medium, incubation is carried out under the same conditions as those described for preparation of inoculum. Samples are taken at intervals, extracted with methyl isobutyl ketone, and the extracts are subjected to paper chromatography on Whatman No. 1 paper with a benzene-ethanol-water solvent system. Steroids containing the u,B-unsaturated ketone function are detected by an ultraviolet scanning device, and the dihydroxyacetone side chain is detected by a blue tetrazolium reagent. In 71 hours the conversion of 9a-fluorohydrocortisone to triamcinolone is complete. No evidence for reduction of the -keto group is seen. The steroid is isolated from the broth by the filtering off the mycelium, extracting the filtrate with isobutyl acetate and concentrating the solvent to dryness, and crystallizing the residue from an acetone-hexane solvent system.

EXAMPLE 2 Vegetative inoculum of the two species, A. simplex and S. roseochromogenes, is prepared as described in Example 1, except that in the second flask stage, 100 ml. of medium C is contained in a 500 ml. Erlenmeyer flask. Inocula so prepared are used to inoculate four liters of Medium D, prepared and sterilized in a 7.5 liter glass fermentor. To the inoculated fermentation broth is added, as soon as possible after inoculation, 2.0 g. of 9a-fluorohydrocortisone suspended in ml. of aqueous 0.01% Tween 80 solution. Incubation temperature (25 is maintained by submerging the fermentor partially in a tempered water bath. Agitation is 400600 r.p.m., aeration is 4 liters/ min. at room temperature.

After 89 hours the conversion of 9a-fluorohydrocortisome to triamcinolone is complete. Quantitative analysis of paper chromatograms shows that the conversion is equal to or better than 90%. The triamcinolone is isolated as in Example 1.

EXAMPLE 3 The two cultures, A. simplex and S. roseochromogenes, are propagated as in Example 1, except that in the second shaken flask stage, 1000 ml. of Medium C is contained in a 4-liter flask equipped with a sidearm transfer tube and inoculating bell. For the fermentation stage, 30 liters of Medium D are prepared and sterilized in a 40-liter stainless steel fermentor provided 'with a jacket for temperature control by means of tempered water, an agitation system, and an aeration system. Immediately after both of the cultures (each 5% vol./vol.) are inoculated into the fermentor, 9.37 g. of 9a-fluorohydrocortisone suspended in 300 ml. of 0.01% aqueous Tween 80 solution is added. Fermentation is carried out at 25 C. with agitation at 220-350 r.p.m. and aeration at 0.51.0 (vol./ vol./min.). Periodic analysis by the paper chromatographic method shows the conversion to triamcinolone to be complete in 81 hours.

The broth is filtered with 5 kg. of Hyflo as filter aid through a Lapp funnel. The mycelial cake is washed on the funnel with about 5 liters of water. Combined filtrate and wash, a total of 41.7 liters, is extracted with a total of 134 liters of methyl isobutyl ketone used in four equal parts in successive extractions. Concentration of the extract to virtual dryness gives 6.02 g. of crude steroid containing 77.8% of triamcinolone. Pure triamcinolone is obtained bymecrystallization from ethanol.

EXAMPLE 4 Following the procedure of Example 1, triamcinolone is produced from 9a-fluorohydrocortisone-21-acetate using S. roseochromogenes and A. Simplex.

EXAMPLE 5 Triamcinolone is produced from 9ot-fluorohydrocorti- .sone-21-hemisuccinate following the procedure of Example 1 using S. roseochromogenes and A. simplex.

EXAMPLE 6 16a-hydroxyprednisolone is produced from hydrocortisone by the procedure of Example 1 using S. roseochromogenes and A. simplex.

EXAMPLE 7 16ot-hydroxyprednisolone-16,17-acetonide is produced from l6a-hydroxycortexolone-16,17-acetonide by following the procedure of Example 1 using Curvularia lunata ATCC No. 12017 and A. simplex.

One ml. of aqueous suspension of C. lunata, grown for two weeks at 25 C. on Medium B, is used to inoculate 50 ml. of Medium C contained in a 250 ml. Erlenmeyer flask. Incubation is carried out at 25 C. with rotary mechanical shaking (280' r.p.m., 1.0 inch radius) for 48 hours. At the same time and under the same conditions, but separately, A. simplex is grown as in Example 1. A second flask stage, in which Medium E m1./ 500 ml.

flask) is employed, is used to propagate the organisms separately for 48 hours under the above conditions. Three flasks of each culture are prepared in the second stage. In the third flask stage 29-500 ml. flasks, each containing 100 ml. of Medium F, are supplemented with 1007 mg. of 16et-hydroxycortexolone-16,17-acetonide suspended in 60 m1. of Tween 80 aqueous solution (2.0 mL/flask). Incubation is for 129 hours under the conditions described above.

The contents of the flasks are pooled and filtered with suction through a Seitz clarifying filter pad. About 870 ml. of distilled water are used to rinse the flasks and wash the mycelial cake. The total volume of filtrate combined with washings is 3570 ml.

This mixture is extracted three times with 1200 m1. portions of water and evaporated under reduced pressure. The residue (1.4 g.) is crystallized from acetone-hexane to give 424 mg. of 16a-hydroxyprednisolone-16,17-acetonide. By thin layer chromatography of the mother liquor using silica gel HF as adsorbent and ethyl acetate chloroform (1:1, v.:v.) as the developing solvent two bands are detectable by UV. light as R 0.2 and 0.5 respectively. By elution of the more polar band and crystallization an additional 64 mg. of 16oc-hydroxypredisolone 16, 17-acetonide is obtained. From the less polar band on elution and crystallization there is obtained 147 mg. of 16 a-hydroxy- 1 -dehydrocortexolone-1 6,17-acetonide.

EXAMPLE 8 l-dehydro-l1a,16a-dihydroxycortexolone is produced from 16a-hydroxycortexolone by the procedure of Example 7 using Aspergillus ochraceus ATCC No. 12337 and A. globiformis ATCC No. 8010. The product is an intermediate in the production of triamcinolone.

EXAMPLE 9 16u-hydroxyprednisolone, an intermediate in the production of triarncinolone, is produced from 16a-hydroxycortexolone by the procedure of Example 8 using Cwrvularia lunata ATCC No. 12017 and A. oxydans, ATCC No. 14349.

EXAMPLE 1O 1-dehydro-l6-dehydro-1la-hydroxycortexone, an intermediate in the production of triamcinolone, is produced from 16-dehydrocortexone-2l-acetate by the procedure of Example 8 using Aspergillus ochraceous and A. ureafaciens ATCC No. 7562.

EXAMPLE 1 l A mixture of l-dehydro-l1a,16m-dihydroxycortexolone-16,17-acetonide and 16u-hydroxyprednisolone-16,17- acetonide, intermediates in the production of triamcinolone, is produced from 16u-hydroxycortexolone-16,17- acetonide-Zl-acetate by the procedure of Example 9 using Absidia Coreulea ATCC No. 14076 and A. simplex.

One ml. of a suspension of surface growth from a 2-week old agar slant culture of A. coerulea on Medium B is used to inoculate 50 ml. of Medium C contained in a 250 ml. Erlenmeyer flask. The inoculated flask is incubated on the rotary shaker (280 cycles/min, 1.0 inch radius) for 48 hours at C. Simultaneously but separately, A. simplex is cultured as in Example 1. Six flasks of Medium B (100 ml./500 ml. flask) are inoculated (three with each culture) in the second pure culture gwowth stage, incubated as in the first. The third flask stage, in which the cultures are mixed is made up of 500 ml. flasks, each containing 100 ml. of Medium F and approximately mg. of l6a-hydroxycortexolone-16,17- acetonide. The steroid is added in suspension in aqueous Tween 80 solution, approximately 2.0 ml./flask, before the flasks are inoculated. A total of 1059 mg. of steroid is added.

The mixed culture fermentation is carried out for hours, the contents of the flasks are pooled, washed with water, filtered with suction on a Seitz clarifying pad, and a total of 3520 ml. of filtrate and washings are collected.

The residual mycelial cake is washed with 900 ml. of acetone which are collected and kept separate from the aqueous filtrate and washings.

The aqueous filtrate and washings are extracted three times with 1200 ml. portions of chloroform. The combined chloroform extracts are washed twice with 2000 ml. portions of water and concentrated under reduced pressure. The residue (1.01 g.) is crystallized from acetone-hexane to give 430 mg. of 16a-hydroxyprednisolone- 16,17-acetonide.

By thin layer chromatography of the mother liquors on silica gel HF using ethyl acetate-chloroform (1:1, v.:v.) as the developing solvent two bands are detectable by UV light at R 0.2 and 0.3 respectively. Elution of the more polar band and crystallization of the residue from acetone-hexane gives 25 mg. of 11u,16a-dihydroxy-1-dehydrocortexolone-16,17-acetonide. From the less polar band on elution and crystallization there are obtained an additional 89 mg. of 16u-hydroxyprednisolone-16,17-acetonide.

Concentration of the acetone washings of the mycelial cake followed by distribution between chloroform and water and evaporation of the chloroform extract gives 161 mg. of residue from which on crystallization by acetone-hexane 50.8 mg. of 16a-hydroxycortexolone-16,17- acetonide are obtained.

EXAMPLE 12 6u-fluoro-16a-hydroxyprednisolone 16,17 acetonide, an intermediate in the production of 6ot-fluorotriamcinolone-16,17-acetonide, is produced from 60L-fil1OIO-160thydroxycortexolone-16,l7-acetonide by the procedure of Example 8 using Cunninghamella blakesleeana ATCC No. 8688a and A. tumescens ATCC No. 6947.

EXAMPLE 13 6a-fluoro-16a-methylprednisolone, an intermediate in the production of 6a-fluorodexamethasone, is produced from 6a-fluoro-16u-methylcortexolone by the procedure of Example 8 using Cunninghamella blakesleeana and A. terregens ATCC No. 13345.

EXAMPLE 14 1-dehydro-17a-hydroxyprogesterone is produced from progesterone by the procedure of Example 7 using A. simplex and T ricothecium roseum.

EXAMPLE 15 1-dehydrodesoxycorticosterone is produced from progesterone by the procedure of Example 7 using A. simplex and Wojnowicia graminis.

What is claimed is:

1. A process for l-dehydrogenating and 16-hydroxylating a seroid which is saturated in the 1,2-position and which has a replaceable hydrogen atom in the 16-position which comprises subjecting said steroid simultaneously to the fermentative action of a l-dehydrogenating bacterium of the genus Arthrobacter and to the fermentative action of a hydroxylating microorganism of the genus Streptomyces in a mixed culture fermentation by adding said steroid and microorganisms or enzymes thereof substantially simultaneously to a medium containing an assim ilable source of carbohydrate, nitrogenous substances, inorganic salts and growth factors, permitting said fermentative actions to take place and recovering the hydroxylated l-dehydro steroid therefrom.

2. A process as in claim 1 wherein the l-dehydrogenator is Arthrobacter simplex and the hydroxylator is Streptomyces roseochromogenes.

3. A process as in claim 2 wherein the starting steroid is 9a-fluorohydrocortisone.

References Cited UNITED OTHER REFERENCES Charney et a1., Microbial Transformations of Steroids, pp. 269 and 684, Academic Press, New York, 1967.

Heftmann et aL, Biochemistry of Steroids, p. 116, Rein- STATES PATENTS 5 hold Publishing Corp., New York, 1960.

M A1 t 1 19551 wz f ig l ALVIN E. TANENHOLTZ, Primary Examiner Wettstein et a1.

Diassi et a1. l. X.R-

Werder et a1. 10 195100, 111 

